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Sequential Injection Analysis System for the Sandwich Hybridization-Based Detection of Nucleic Acids

机译:基于夹心杂交的核酸序列注入分析系统

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摘要

A sequential injection analysis lab-on-valve (SIA-LOV) system was developed for the specific detection of single-stranded nucleic acid sequences via sandwich hybridization of specific DNA probes to the target sequence. One DNA probe was tagged with fluorescein; the other was biotinylated and immobilized to streptavidin-coated porous beads. The system was optimized with respect to buffer composition, length of hybridization and wash steps, and volumes and concentrations of components used. On-bead oligonucleotide hybridization was studied using UV detection at 260 nm, while a final dose response curve was quantified using fluorescence detection. A dynamic range of 1-1000 pmol was obtained for a synthetic DNA sequence that was homologous to a segment in the B. anthracis atxA mRNA. A within-day variation of 7.2percent and a day-to-day variation of 9.9percent was observed. Each analysis was completed within 20 min. Subsequently, the system was applied to the detection of atxA mRNA expressed in a surrogate organism and amplified using NASBA. The SIA-LOV will find its application in routine laboratory-based analysis of specific single-stranded DNA/RNA sequences. Future improvements will include the integration of dye-encapsulating liposomes for signal enhancement used in lieu of the single fluorophore-labeled probe in order to lower the limit of detection.
机译:开发了一种顺序注射分析阀上实验室(SIA-LOV)系统,用于通过特定DNA探针与目标序列的夹心杂交来特异性检测单链核酸序列。一根DNA探针标记有荧光素;另一个被生物素化并固定在链霉亲和素包被的多孔珠上。关于缓冲液组成,杂交和洗涤步骤的长度以及所用组分的体积和浓度,对该系统进行了优化。使用260 nm的UV检测研究珠上寡核苷酸杂交,同时使用荧光检测定量最终剂量反应曲线。对于与炭疽芽孢杆菌atxA mRNA中的一个片段同源的合成DNA序列,获得了1-1000pmol的动态范围。观察到日内变化为7.2%,每日变化为9.9%。每次分析均在20分钟内完成。随后,将该系统应用于检测在替代生物中表达的atxA mRNA,并使用NASBA进行扩增。 SIA-LOV将在常规的基于实验室的特定单链DNA / RNA序列分析中得到应用。未来的改进将包括染料封装脂质体的集成,以代替单个荧光团标记的探针来增强信号,从而降低检测限。

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